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首页> 外文期刊>Nucleic acids research >A rapid and efficient method to generate multiple gene disruptions in Dictyostelium discoideum using a single selectable marker and the Cre-loxP system
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A rapid and efficient method to generate multiple gene disruptions in Dictyostelium discoideum using a single selectable marker and the Cre-loxP system

机译:使用单个选择标记和Cre-loxP系统快速有效地在Disciostelium Discoideum中产生多个基因破坏的方法

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Dictyostelium discoideum has proven an exceptionally powerful system for studying numerous aspects of cellular and developmental functions. The relatively small (~34 Mb) chromosomal genome of Dictyostelium and high efficiency of targeted gene disruption have enabled researchers to characterize many specific gene functions. However, the number of selectable markers in Dictyostelium is restricted, as is the ability to perform effective genetic crosses between strains. Thus, it has been difficult to create multiple mutations within an individual cell to study epistatic relationships among genes or potential redundancies between various pathways. We now describe a robust system for the production of multiple gene mutations in Dictyostelium by recycling a single selectable marker, Blasticidin S resistance, using the Cre-loxP system. We confirm the effectiveness of the system by generating a single cell carrying four separate gene disruptions. Furthermore, the cells remain sensitive to transformation for additional targeted or random mutagenesis requiring Blasticidin selection and for functional expression studies of mutated or tagged proteins using other selectable markers.
机译:Dictyostelium discoideum已被证明是一种功能强大的系统,可用于研究细胞和发育功能的各个方面。 Dictyostelium的染色体基因组相对较小(〜34 Mb),并且靶向基因破坏效率高,这使得研究人员能够表征许多特定的基因功能。然而,双歧杆菌中选择标记的数量受到限制,在菌株之间进行有效遗传杂交的能力也受到限制。因此,很难在单个细胞内产生多个突变来研究基因之间的上位关系或各种途径之间的潜在冗余。我们现在描述一个健壮的系统,用于通过使用Cre-loxP系统回收单个选择标记Blasticidin S抗性,在盘基网柄菌中产生多个基因突变。我们通过产生携带四个单独的基因破坏的单个细胞来确认系统的有效性。此外,对于需要进行弹力素选择的其他靶向或随机诱变以及使用其他选择标记进行的突变或标记蛋白的功能性表达研究,细胞仍然对转化敏感。

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